Sexual and asexual re57773-63-4 cost production [15],Evolution of Virulence and Fungicide Resistance[16]. Wind-dispersed ascospores produced by the teleomorph contribute significantly both to initiation and further development of disease epidemics [18] and are likely to be one of the main mechanisms contributing to long distance gene flow [19] and host adaptation [20]. Genetic variation in M. graminicola populations is high [21] as a result of frequent sexual recombination [18], [20], high gene flow [22] and large effective population size [22]. Results from experimental evolution and population genetic studies indicate that the genetic structure of the pathogen can change significantly over a single growing season in response to host selection [23], while local adaptation leads to significant population differentiation for virulence [24], fungicide resistance [25] and temperature sensitivity [26]. Though both quantitative and qualitative resistances have been identified in wheat hosts, the majority of resistant cultivars used in commercial production Avasimibe custom synthesis display quantitative resistance (QR) to the pathogen [27], [28]. QR is believed to be more durable because natural selection is thought to operate more slowly on quantitative traits. Unlike qualitative resistance (also called major gene resistance), QR is thought to be mediated by several genes each contributing small but additive effects to the overall host resistance [29]. It is thought that mechanisms underlying QR in plants involve preformed, constitutive, physical and chemical barriers, Pathogen-Associated Molecular Pattern (PAMP)-triggered responses [5] and pathogen life-history traits [30]. Interactions of these mechanisms hinder the growth, penetration, reproduction and transmission of a pathogen. QR in plants slows down but does not prevent epidemics, thus effective disease control may require supplementary applications of fungicides. Triazoles represent a major category of fungicides used widely in agriculture and medicine. This group of fungicides inhibits cytochrome P450 sterol 14 alpha-demethylase, an enzyme required for the biosynthesis of ergosterol in many fungi [31]. Resistance to triazoles is thought to be polygenic [32] and mediated by several mechanisms including mutations in the target protein gene CYP51 and increased active efflux by ABC transporters [33], [34], [35], [36]. Cyproconazole is a triazole fungicide that has been used for many years to control M. graminicola [32].The genotype data were published earlier [21]. Only isolates with a distinct multi-locus RFLP haplotype and DNA fingerprint were chosen for virulence and fungicide resistance tests. A total of 141 genetically distinct isolates were included in the experiment. Each population was represented by 25?0 isolates.Measurement of cyproconazole toleranceM. graminicola isolates retrieved from silica gel long-term storage were grown on potato dextrose agar (PDA) amended with 50 mg/ L kanamycin and placed at 18uC for seven days. Blastospores formed on these plates were transferred into 50 mL Falcon tubes containing 30 ml 16574785 yeast sucrose broth (YSB) supplemented with 50 mg/L kanamycin. The tubes were placed at 18uC at 140 rpm for seven days. Spore concentrations for each isolate were determined on the day of inoculation using a haemocytometer and adjusted to 200 spores per mL. 500 mL of the calibrated spore suspension was inoculated onto a PDA plate containing 0.1 ppm cyproconazole while another 500 mL of the spore suspension.Sexual and asexual reproduction [15],Evolution of Virulence and Fungicide Resistance[16]. Wind-dispersed ascospores produced by the teleomorph contribute significantly both to initiation and further development of disease epidemics [18] and are likely to be one of the main mechanisms contributing to long distance gene flow [19] and host adaptation [20]. Genetic variation in M. graminicola populations is high [21] as a result of frequent sexual recombination [18], [20], high gene flow [22] and large effective population size [22]. Results from experimental evolution and population genetic studies indicate that the genetic structure of the pathogen can change significantly over a single growing season in response to host selection [23], while local adaptation leads to significant population differentiation for virulence [24], fungicide resistance [25] and temperature sensitivity [26]. Though both quantitative and qualitative resistances have been identified in wheat hosts, the majority of resistant cultivars used in commercial production display quantitative resistance (QR) to the pathogen [27], [28]. QR is believed to be more durable because natural selection is thought to operate more slowly on quantitative traits. Unlike qualitative resistance (also called major gene resistance), QR is thought to be mediated by several genes each contributing small but additive effects to the overall host resistance [29]. It is thought that mechanisms underlying QR in plants involve preformed, constitutive, physical and chemical barriers, Pathogen-Associated Molecular Pattern (PAMP)-triggered responses [5] and pathogen life-history traits [30]. Interactions of these mechanisms hinder the growth, penetration, reproduction and transmission of a pathogen. QR in plants slows down but does not prevent epidemics, thus effective disease control may require supplementary applications of fungicides. Triazoles represent a major category of fungicides used widely in agriculture and medicine. This group of fungicides inhibits cytochrome P450 sterol 14 alpha-demethylase, an enzyme required for the biosynthesis of ergosterol in many fungi [31]. Resistance to triazoles is thought to be polygenic [32] and mediated by several mechanisms including mutations in the target protein gene CYP51 and increased active efflux by ABC transporters [33], [34], [35], [36]. Cyproconazole is a triazole fungicide that has been used for many years to control M. graminicola [32].The genotype data were published earlier [21]. Only isolates with a distinct multi-locus RFLP haplotype and DNA fingerprint were chosen for virulence and fungicide resistance tests. A total of 141 genetically distinct isolates were included in the experiment. Each population was represented by 25?0 isolates.Measurement of cyproconazole toleranceM. graminicola isolates retrieved from silica gel long-term storage were grown on potato dextrose agar (PDA) amended with 50 mg/ L kanamycin and placed at 18uC for seven days. Blastospores formed on these plates were transferred into 50 mL Falcon tubes containing 30 ml 16574785 yeast sucrose broth (YSB) supplemented with 50 mg/L kanamycin. The tubes were placed at 18uC at 140 rpm for seven days. Spore concentrations for each isolate were determined on the day of inoculation using a haemocytometer and adjusted to 200 spores per mL. 500 mL of the calibrated spore suspension was inoculated onto a PDA plate containing 0.1 ppm cyproconazole while another 500 mL of the spore suspension.
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